Structural basis for antigenic peptide precursor processing by the endoplasmic reticulum aminopeptidase ERAP1

Nguyen, Truyen; Chang, Shih‐Chung; Evnouchidou, Irini; York, Ian A.; Zikos, Christos; Rock, Kenneth L.; Goldberg, Alfred L.; Stratikos, Efstratios; Stern, Lawrence J.

doi:10.1038/nsmb.2021

Cited by 184 publications

(387 citation statements)

References 58 publications

(101 reference statements)

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“…The latter feature refers to the low ERAP1-trimming activity toward most peptides shorter than eight residues (12,16). Absence of ERAP activity has been shown to drastically change the profile of MHC class I-associated peptides (17) and/or alter Ag presentation in vitro and in vivo in numerous experimental systems (18)(19)(20).…”

Section: P Rocessing Of Ags For Presentation By Mhc Proteins Involvesmentioning

confidence: 99%

“…ERAP1 crystallizes as a trimer and ERAP2 as a dimer. Interestingly, the interaction sites in these multimers correspond to residues conserved between the two enzymes (16,21). However, the functional significance of dimer formation for ERAP-trimming activity remains unknown.…”

Section: P Rocessing Of Ags For Presentation By Mhc Proteins Involvesmentioning

confidence: 99%

“…ERAP1 has been shown to possess regulatory sites different from the active site that modulates its activity (16). Dimerization might represent an additional level of allosteric regulation.…”

Section: Heterodimerization Changes Basic Enzymatic Parametersmentioning

confidence: 99%

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ERAP1–ERAP2 Dimerization Increases Peptide-Trimming Efficiency

Evnouchidou

Weimershaus

Saveanu

et al. 2014

The Journal of Immunology

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The endoplasmic reticulum aminopeptidases (ERAP)1 and ERAP2 play a critical role in the production of final epitopes presented by MHC class I molecules. Formation of heterodimers by ERAP1 and ERAP2 has been proposed to facilitate trimming of epitope precursor peptides, but the effects of dimerization on ERAP function remain unknown. In this study, we produced stabilized ERAP1–ERAP2 heterodimers and found that they produced several mature epitopes more efficiently than a mix of the two enzymes unable to dimerize. Physical interaction with ERAP2 changes basic enzymatic parameters of ERAP1 and improves its substrate-binding affinity. Thus, by bringing the two enzymes in proximity and by producing allosteric effects on ERAP1, dimerization of ERAP1/2 creates complexes with superior peptide-trimming efficacy. Such complexes are likely to enhance Ag presentation by cells displaying coordinated expression of the two enzymes.

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Section: P Rocessing Of Ags For Presentation By Mhc Proteins Involvesmentioning

confidence: 99%

Section: P Rocessing Of Ags For Presentation By Mhc Proteins Involvesmentioning

confidence: 99%

See 1 more Smart Citation

ERAP1–ERAP2 Dimerization Increases Peptide-Trimming Efficiency

Evnouchidou

Weimershaus

Saveanu

et al. 2014

The Journal of Immunology

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“…The crystal structure of ERAP1 (bound to bestatin) reveals a large cavity that would explain the preference for longer substrates compared to most other aminopeptidases (Nguyen, Chang et al 2011). In this large cavity a catalytic site is found to which the Nterminal part of the peptide binds.…”

Section: Erap Aminopeptidases Trim Er Peptides To Fit the Mhc-i Peptimentioning

confidence: 99%

“…It has been proposed that in close proximity to this catalytic site a regulatory site is found to which the C-terminal part of the peptide is bound, this "double binding" ensures a closed conformation of the ERAP1 molecule resulting in effective cleaving of the peptide. However, if the peptide is too short the C-terminal will not reach the regulatory site and the "double binding" will not be achieved resulting in an ineffective cleaving of the peptide (Nguyen, Chang et al 2011). …”

Section: Erap Aminopeptidases Trim Er Peptides To Fit the Mhc-i Peptimentioning

confidence: 99%

MHC Class I Quality Control

Røder

Ulfsson²,

Follin³

et al. 2012

Histocompatibility

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Dominant Role of the ERAP1 Polymorphism R528K in Shaping the HLA–B27 Peptidome Through Differential Processing Determined by Multiple Peptide Residues

Sanz-Bravo

Campos

Mazariegos

et al. 2015

Arthritis & Rheumatology

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Objective. To characterize the alterations, as well as their mechanisms, induced in the HLA-B27-bound peptidome expressed in live cells by the natural ERAP1 polymorphisms predisposing to ankylosing spondylitis (AS): R528K and N575D/Q725R.Methods. HLA-B*27:05-bound peptides were isolated from 3 human lymphoid cell lines expressing distinct ERAP1 variants differing at residues 528 and/or 575/725. The high-performance liquid chromatographyfractionated peptide pools were compared by mass spectrometry based on identity of molecular mass and chromatographic retention time. The relative amount of each shared peptide in any given cell line pair was estimated from the respective ion peak intensities. Peptide sequencing was also carried out by mass spectrometry.Results. HLA-B27-bound ligands predominant in the context of the ERAP1 variant with K528 collectively showed higher molecular mass, higher frequency of N-terminal residues resistant to ERAP1, and bulkier residues downstream of the N-terminus, relative to peptides predominant in the R528 context. None of these differences were observed with ERAP1 variants differing at positions 575/725, but not at residue 528. Neither R528K nor N575D/Q725R altered the mean length of B*27:05-bound ligands.Conclusion. The R528K, but not the N575D/ Q725R, polymorphism alters the expression levels of many HLA-B*27:05-bound peptides, depending on the susceptibility of their N-terminal residues to trimming and depending on the size of the amino acid side chains at multiple positions downstream of the N-terminus. The significant alterations in the B*27:05 peptidome and the structural features of the peptides that determine their differential expression in distinct ERAP1 contexts account for the association of the R528K polymorphism with AS.

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Structural basis for antigenic peptide precursor processing by the endoplasmic reticulum aminopeptidase ERAP1

Cited by 184 publications

References 58 publications

ERAP1–ERAP2 Dimerization Increases Peptide-Trimming Efficiency

ERAP1–ERAP2 Dimerization Increases Peptide-Trimming Efficiency

MHC Class I Quality Control

Dominant Role of the ERAP1 Polymorphism R528K in Shaping the HLA–B27 Peptidome Through Differential Processing Determined by Multiple Peptide Residues

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